GENERATION OF A FAMILY OF PROTEIN-FRAGMENTS FOR STRUCTURE-FOLDING STUDIES .1. FOLDING COMPLEMENTATION OF 2 FRAGMENTS OF CHYMOTRYPSIN INHIBITOR-2 FORMED BY CLEAVAGE AT ITS UNIQUE METHIONINE RESIDUE

被引:63
作者
GAY, GD [1 ]
FERSHT, AR [1 ]
机构
[1] UNIV CAMBRIDGE,DEPT CHEM,MRC,PROT FUNCT & DESIGN UNIT,CAMBRIDGE CB2 1EW,ENGLAND
来源
BIOCHEMISTRY | 1994年 / 33卷 / 25期
关键词
D O I
10.1021/bi00191a024
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The suitability of the barley chymotrypsin inhibitor-2 for study by fragmentation and complementation has been analyzed. The primary residue for binding to proteases, Met-59 (the unique methionine in the sequence), lies in a broad, solvent-exposed loop. The bond between Met-59 and Glu-60 was cleaved by cyanogen bromide. The two fragments thus obtained, i.e., CI-2(20-59) and CI-2(60-83), associate (K-D = 42 nM) to yield a complex that has fluorescence and circular dichroism spectra identical to those of uncleaved chymotrypsin inhibitor-2. Recovery of native-like structure is further indicated by the ability of the complex to inhibit chymotrypsin, although the [I]50% is 140-fold higher than for the uncleaved inhibitor. CI-2(60-83) appears to be highly disordered in water, but fragment CI(20-59) forms significative structure, as judged by its circular dichroism spectra and evidence from one-dimensional NMR. The circular dichroism spectra of CI-2(20-59) approach the baseline in 4 M guanidinium chloride but display characteristics of an or-helix in the presence of trifluoroethanol. Analytical ultracentrifugation shows no concentration-dependent change in the molecular weight of the monomer of CI-2(20-59). Both one- and two-dimensional NMR of the complex [CI-2(20-59).(60-83)] show unequivocally the presence of a folded structure, which appears to be slightly different from the uncleaved native protein.
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页码:7957 / 7963
页数:7
相关论文
共 30 条
[1]  
Anfinsen C B, 1975, Adv Protein Chem, V29, P205, DOI 10.1016/S0065-3233(08)60413-1
[2]   HELIX-COIL TRANSITION OF ISOLATED AMINO TERMINUS OF RIBONUCLEASE [J].
BROWN, JE ;
KLEE, WA .
BIOCHEMISTRY, 1971, 10 (03) :470-&
[3]   DETERMINATION OF THE AGGREGATE SIZE IN DETERGENT SOLUTION OF THE LIGHT-HARVESTING CHLOROPHYLL A/B-PROTEIN COMPLEX FROM CHLOROPLAST MEMBRANES [J].
BUTLER, PJG ;
KUHLBRANDT, W .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1988, 85 (11) :3797-3801
[4]   THERMODYNAMIC ANALYSIS OF MULTICOMPONENT SOLUTIONS [J].
CASASSA, EF ;
EISENBERG, H .
ADVANCES IN PROTEIN CHEMISTRY, 1964, 19 :287-395
[5]   DETERMINATION OF SECONDARY STRUCTURES OF PROTEINS BY CIRCULAR-DICHROISM AND OPTICAL ROTATORY DISPERSION [J].
CHEN, YH ;
YANG, JT ;
MARTINEZ, HM .
BIOCHEMISTRY, 1972, 11 (22) :4120-+
[6]   THE DETERMINATION OF THE 3-DIMENSIONAL STRUCTURE OF BARLEY SERINE PROTEINASE INHIBITOR-2 BY NUCLEAR-MAGNETIC-RESONANCE, DISTANCE GEOMETRY AND RESTRAINED MOLECULAR-DYNAMICS [J].
CLORE, GM ;
GRONENBORN, AM ;
KJAER, M ;
POULSEN, FM .
PROTEIN ENGINEERING, 1987, 1 (04) :305-311
[7]   FOLDING OF PEPTIDE-FRAGMENTS COMPRISING THE COMPLETE SEQUENCE OF PROTEINS - MODELS FOR INITIATION OF PROTEIN FOLDING .2. PLASTOCYANIN [J].
DYSON, HJ ;
SAYRE, JR ;
MERUTKA, G ;
SHIN, HC ;
LERNER, RA ;
WRIGHT, PE .
JOURNAL OF MOLECULAR BIOLOGY, 1992, 226 (03) :819-835
[8]  
DYSON HJ, 1991, ANNU REV BIOPHYS BIO, V20, P519
[9]   FOLDING OF PEPTIDE-FRAGMENTS COMPRISING THE COMPLETE SEQUENCE OF PROTEINS - MODELS FOR INITIATION OF PROTEIN FOLDING .1. MYOHEMERYTHRIN [J].
DYSON, HJ ;
MERUTKA, G ;
WALTHO, JP ;
LERNER, RA ;
WRIGHT, PE .
JOURNAL OF MOLECULAR BIOLOGY, 1992, 226 (03) :795-817
[10]  
GAY GD, 1994, BIOCHEMISTRY-US, V32, P7964
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